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大鼠肾上腺细胞中洋地黄样化合物的生物合成:羟基胆固醇作为可能的前体。

Biosynthesis of digitalis-like compounds in rat adrenal cells: hydroxycholesterol as possible precursor.

作者信息

Lichtstein D, Steinitz M, Gati I, Samuelov S, Deutsch J, Orly J

机构信息

Department of Physiology, The Hebrew University-Hadassah Medical School, Jerusalem, Israel.

出版信息

Life Sci. 1998;62(23):2109-26. doi: 10.1016/s0024-3205(98)00186-6.

Abstract

The biosynthesis of digitalis-like compounds (DLC) was determined in bovine and rat adrenal homogenates, as well as in primary rat adrenal cells, by following changes in the concentration of DLC using three independent sensitive bioassays: inhibition of [3H]-ouabain binding to red blood cells and competitive ouabain and bufalin ELISA. The amounts of DLC in bovine and rat adrenal homogenates, as measured by the two first bioassays, increased with time when the mixtures were incubated under tissue culture conditions. Rat primary adrenal cells were incubated in the presence of [1,2-(3)H]-25-hydroxycholesterol, [26,27-(3)H]-25-hydroxycholesterol or [7-(3)H]-pregnenolone. The radioactive products, as well as the digitalis-like activity, were fractionated by three sequential chromatography systems. When [1,2-(3)H]-25-hydroxycholesterol or [7-(3)H]-pregnenolone was added to the culture medium, the radioactivity was co-eluted with digitalis-like activity, suggesting that at least one of the DLC might originate in hydroxycholesterol. In contrast, when the culture medium was supplemented with [26,27-(3)H]-25-hydroxycholesterol, the radioactivity was not co-eluted with the digitalis-like activity, indicating that side chain cleavage is the first step in the synthesis of digitalis-like compounds by rat adrenal.

摘要

通过使用三种独立的灵敏生物测定法跟踪洋地黄样化合物(DLC)浓度的变化,来测定牛和大鼠肾上腺匀浆以及原代大鼠肾上腺细胞中DLC的生物合成:抑制[³H]-哇巴因与红细胞的结合以及竞争性哇巴因和蟾毒灵酶联免疫吸附测定。当混合物在组织培养条件下孵育时,通过前两种生物测定法测得的牛和大鼠肾上腺匀浆中DLC的量随时间增加。将原代大鼠肾上腺细胞在[1,2-(³H)]-25-羟胆固醇、[26,27-(³H)]-25-羟胆固醇或[7-(³H)]-孕烯醇酮存在的情况下孵育。放射性产物以及洋地黄样活性通过三个连续的色谱系统进行分离。当向培养基中添加[1,2-(³H)]-25-羟胆固醇或[7-(³H)]-孕烯醇酮时,放射性与洋地黄样活性共洗脱,表明至少一种DLC可能起源于羟胆固醇。相反,当培养基中添加[26,27-(³H)]-25-羟胆固醇时,放射性与洋地黄样活性未共洗脱,表明侧链裂解是大鼠肾上腺合成洋地黄样化合物的第一步。

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